Difference between revisions of "Project:Plant species testing"

Revision as of 19:27, 21 July 2012

We are using primers for plants to test and refine our DNA extraction / PCR technique. First project is to test for peas. Inspiration and primers are in this paper. We are using two methods of extraction. 1st attempt with a chelex protocol, 2nd with alcohol precipitation.

1st go - 17 and 18/7/12

Extraction (From this paper - we also have full text available):

'Homogenize' (mush) approx 40 mg pea with a pestle in 300ul of 5% chelex solution for 1 min
Vortex for 10s then boil for 5 mins, then vortex again for 10s. (Hot plate lost heat in the middle so we boiled for 8 mins)
Centrifuge for 1 min - recover supernatant and use as template

PCR:

Prepare sample with 12.5 ul of Taq ready mix, 2 ul of each primer, 3 ul of template, and 5.5 ul of distilled water.
Denature at 96°C for 5 mins
40 cycles of D = 96°C for one minute, A = 58°C for 30 seconds, E = 72°C for one minute.
Put paraffin on top after 5 mins (should have been before start)

Electrophoresis:

100ml of agarose solution: 1 gram of agarose powder added to 100ml of 1% TBE solution
Microwaved the agarose, cooled to 50 degrees, added 5ul of ethidium bromide stock solution
Poured agarose into mould and waited to cool, then covered with 1% TBE.
Put ladder into far well, template into near well
Electrophoresed for 1 hr - started at 80V, settled at around 130V
Visualised under UV light through orange filter - did not see any bands from the template, but ladder was visible, indicating PCR failed.

Repeat without PCR

Extraction:

'Homogenize' (mush) approx 50 mg pea with a disposable pipette tube in 600ul of 5% chelex solution for 1 min
Vortex for 10s then boil for 5 mins, then vortex again for 10s.
Centrifuge for 1 min - recover supernatant and use as template

Electrophoresis:

100ml of agarose solution: 1 gram of agarose powder added to 100ml of 1% TBE solution
Microwaved the agarose, cooled to 50 degrees, added 5ul of ethidium bromide stock solution
Poured agarose into mould and waited to cool, then covered with 1% TBE.
Put ladder into far well, template into near well
Electrophoresed for 1 hr at 80V
Visualised under UV light through orange filter - saw a faint, blurry band, running ahead of the ladder, which we assumed to be the genomic DNA we were looking for.

2nd go

Blend peas with salt and detergent according to this protocol. Sieve.
Incubate for 15 mins at 60°C (optional step that we didn't take)
Centrifuge - recover supernatant
Add proteinease K (100 ul of 1mg / ml solution to 300 ul of pea template) - incubate for 1 hr at 50C (action of proteinase k) then 94 C for 10 mins (inactivation of proteinase K)
Precipitation to follow

@@ Line 24: / Line 24: @@
 * Electrophoresed for 1 hr - started at 80V, settled at around 130V
 * Visualised under UV light through orange filter - did not see any bands from the template, but ladder was visible, indicating PCR failed.
+==== Repeat without PCR ====
+Extraction:
+* 'Homogenize' (mush) approx 50 mg pea with a disposable pipette tube in 600ul of 5% chelex solution for 1 min
+* Vortex for 10s then boil for 5 mins, then vortex again for 10s.
+* Centrifuge for 1 min - recover supernatant and use as template
+Electrophoresis:
+* 100ml of agarose solution: 1 gram of agarose powder added to 100ml of 1% TBE solution
+* Microwaved the agarose, cooled to 50 degrees, added 5ul of ethidium bromide stock solution
+* Poured agarose into mould and waited to cool, then covered with 1% TBE.
+* Put ladder into far well, template into near well
+* Electrophoresed for 1 hr at 80V
+* Visualised under UV light through orange filter - saw a faint, blurry band, running ahead of the ladder, which we assumed to be the genomic DNA we were looking for.
 == 2nd go ==

Difference between revisions of "Project:Plant species testing"

Revision as of 19:27, 21 July 2012

1st go - 17 and 18/7/12

Repeat without PCR

2nd go

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